AI Article Synopsis

  • Retinal degenerative diseases lead to irreversible loss of photoreceptors, with cell replacement therapy being a promising treatment approach.
  • Müller glia in the retina can serve as source cells due to their ability to revert to a progenitor-like state, showing characteristics like stem cell markers and self-renewal potential.
  • Research identified that the microRNA miR-28 negatively regulates CRX, a key transcription factor for photoreceptors; inhibiting miR-28 promotes differentiation of Müller glia-derived progenitors into neurons expressing photoreceptor-specific proteins, suggesting a potential pathway for treatment.

Article Abstract

Retinal degenerative diseases ultimately result into irreversible photoreceptor death or loss. At present, the most promising treatment for these diseases is cell replacement therapy. Müller glia are the major glia in the retina, displaying cardinal features of retinal progenitor cells, and can be candidate of seed cells for retinal degenerative diseases. Here, mouse retinal Müller glia dissociated and cultured in vitro amplified and were dedifferentiated into Müller glia-derived progenitors (MGDPs), demonstrating expression of stem/progenitor cell markers Nestin, Sox2 and self-renewal capacity. MicroRNAs (miRNAs) play unique roles in the retinogenesis, so we hypothesized miRNAs would contribute to photoreceptor lineage commitment of MGDPs. By TargetScan, Miranda, and Pictar bioinformatics, gain/loss-of-function models, dual luciferase assay, we identified and validated that miR-28 targeted the photoreceptor-specific CRX transcription factor. Anti-miR-28 could induce MGDPs to differentiate into neurons strongly expressing CRX and Rhodopsin, while miR-28 mimic suppressed CRX and Rhodopsin expression. Knockdown of CRX by siRNA blocked the expression of CRX and Rhodospin upregulated by anti-miR-28, indicating that anti-miR-28 potentially induced photoreceptor commitment of MGDPs by targeting CRX, but more experiments are necessary to confirm their role in differentiation.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC5595954PMC
http://dx.doi.org/10.1038/s41598-017-11112-4DOI Listing

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